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Delayed luminescence of Prorocentrum minimum under controlled conditions
Authors:Marina Monti   Alexis Zrimec   Alfred Beran   Maja Berden Zrimec   Luka Drinovec   Gorazd Kosi  Francesco Tamberlich
Affiliation:aLaboratory of Marine Biology, Via Auguste Piccard 54, I-34010 Trieste, Italy;bInstitute of Physical Biology, Velika Loka 90, SI-1290 Grosuplje, Slovenia;cNational Institute of Biology, Večna pot 111, SI-1000 Ljubljana, Slovenia
Abstract:
Delayed luminescence (DL), also termed delayed fluorescence or delayed light emission, is the phenomenon of long-lived light emission by plants and cyanobacteria after being illuminated with light and put into darkness. Culture growth of three Prorocentrum minimum strains was studied with DL measurements. DL decay kinetics was measured from 1–60 s after a pulse of white light. The strains used were from the Adriatic Sea (PmK), from Chesapeake Bay, USA (D5), and from the Baltic Sea (BAL), cultured at salinity of 32, 16, and 8 (practical salinity scale), respectively. The strains differed in cell size and chlorophyll a content (PmK > D5 > BAL), as well as in DL parameters. The DL results were compared to standard measurements of culture density and carbon content (calculated from biovolumes). DL decay curves had a specific peak, which changed with culture growth and showed more similarities between the strains PmK and D5. The DL intensity increased with cell density and carbon content in a two-stage process, corresponding to the lag and exponential phases of growth. DL intensity was best correlated with carbon content irrespective of strain and is proposed as an estimate of biomass and for differentiating between lag and exponential phases of growth.
Keywords:Prorocentrum minimum   Delayed luminescence   Growth phases
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